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保守基序中的突变会抑制噬菌体T4 UvsY蛋白的单链DNA结合及重组介导活性。

Mutations in a conserved motif inhibit single-stranded DNA binding and recombination mediator activities of bacteriophage T4 UvsY protein.

作者信息

Bleuit Jill S, Ma Yujie, Munro James, Morrical Scott W

机构信息

Departments of Biochemistry and Microbiology and Molecular Genetics, University of Vermont College of Medicine, Burlington, Vermont 05405, USA.

出版信息

J Biol Chem. 2004 Feb 13;279(7):6077-86. doi: 10.1074/jbc.M311557200. Epub 2003 Nov 22.

DOI:10.1074/jbc.M311557200
PMID:14634008
Abstract

The UvsY recombination mediator protein is critical for homologous recombination in bacteriophage T4. UvsY uses both protein-protein and protein-DNA interactions to mediate the assembly of the T4 UvsX recombinase onto single-stranded (ss) DNA, forming presynaptic filaments that initiate DNA strand exchange. UvsY helps UvsX compete with Gp32, the T4 ssDNA-binding protein, for binding sites on ssDNA, in part by destabilizing Gp32-ssDNA interactions, and in part by stabilizing UvsX-ssDNA interactions. The relative contributions of UvsY-ssDNA, UvsY-Gp32, UvsY-UvsX, and UvsY-UvsY interactions to these processes are only partially understood. The goal of this study was to isolate mutant forms of UvsY protein that are specifically defective in UvsY-ssDNA interactions, so that the contribution of this activity to recombination processes could be assessed independent of other factors. A conserved motif of UvsY found in other DNA-binding proteins was targeted for mutagenesis. Two missense mutants of UvsY were isolated in which ssDNA binding activity is compromised. These mutants retain self-association activity, and form stable associations with UvsX and Gp32 proteins in patterns similar to wild-type UvsY. Both mutants are partially, but not totally, defective in stimulating UvsX-catalyzed recombination functions including ssDNA-dependent ATP hydrolysis and DNA strand exchange. The data are consistent with a model in which UvsY plays bipartite roles in presynaptic filament assembly. Its protein-ssDNA interactions are suggested to moderate the destabilization of Gp32-ssDNA, whereas its protein-protein contacts induce a conformational change of the UvsX protein, giving UvsX a higher affinity for the ssDNA and allowing it to compete more effectively with Gp32 for binding sites.

摘要

UvsY重组介导蛋白对噬菌体T4中的同源重组至关重要。UvsY利用蛋白质-蛋白质和蛋白质-DNA相互作用来介导T4 UvsX重组酶在单链(ss)DNA上的组装,形成启动DNA链交换的突触前细丝。UvsY帮助UvsX与T4单链DNA结合蛋白Gp32竞争单链DNA上的结合位点,部分是通过破坏Gp32-ssDNA相互作用,部分是通过稳定UvsX-ssDNA相互作用。UvsY-ssDNA、UvsY-Gp32、UvsY-UvsX和UvsY-UvsY相互作用对这些过程的相对贡献仅得到部分理解。本研究的目标是分离出在UvsY-ssDNA相互作用中存在特异性缺陷的UvsY蛋白突变形式,以便能够独立于其他因素评估该活性对重组过程的贡献。在其他DNA结合蛋白中发现的UvsY保守基序被作为诱变靶点。分离出了两个UvsY错义突变体,其单链DNA结合活性受损。这些突变体保留了自我缔合活性,并以与野生型UvsY相似的模式与UvsX和Gp32蛋白形成稳定缔合。两个突变体在刺激UvsX催化的重组功能(包括单链DNA依赖性ATP水解和DNA链交换)方面都存在部分但非完全缺陷。数据与一个模型一致,即UvsY在突触前细丝组装中起双重作用。其蛋白质-ssDNA相互作用被认为可缓和Gp32-ssDNA的去稳定化,而其蛋白质-蛋白质接触诱导UvsX蛋白的构象变化,使UvsX对单链DNA具有更高的亲和力,并使其能够更有效地与Gp32竞争结合位点。

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